Simplified detection of a mutation causing familial hypercholesterolaemia throughout Britain: evidence for an origin in a common distant ancestor

P R Wenham; L Haddad; M Panarelli; J P Ashby; I N Day; P D Giles; S E Humphries; M D Penney; P W Rae; S W Walker

doi:10.1177/000456329803500205

Simplified detection of a mutation causing familial hypercholesterolaemia throughout Britain: evidence for an origin in a common distant ancestor

Ann Clin Biochem. 1998 Mar:35 ( Pt 2):226-35. doi: 10.1177/000456329803500205.

Authors

P R Wenham¹, L Haddad, M Panarelli, J P Ashby, I N Day, P D Giles, S E Humphries, M D Penney, P W Rae, S W Walker

Affiliation

¹ Department of Clinical Biochemistry, Western General Hospital, Edinburgh, UK.

PMID: 9547893
DOI: 10.1177/000456329803500205

Abstract

Familial hypercholesterolaemia (FH) is an inherited autosomal codominant disorder caused by many different mutations in the low-density lipoprotein receptor (LDLR) gene. The one described most frequently in patients with FH from England, arises from a G-->A transition at the first nucleotide of codon 80, resulting in the substitution of lysine for glutamic acid at residue 80 of the mature protein, FH E80K. We describe a simple method to detect this mutation in genomic DNA using the polymerase chain reaction (PCR). A 69 base pair (bp) fragment of exon 3 of the LDLR gene is amplified using a mutagenic upstream PCR primer. This substitutes a T for an A residue in the amplified product, 2 bp upstream from the mutant site, generating a restriction site for the endonuclease Taq I, in normal, but not in mutant DNA. Following digestion of amplified DNA with Taq I, normal but not mutant DNA is cut into two fragments of 29 and 40 bp, which are readily identified by polyacrylamide gel electrophoresis. Using this method, 410 patients with clinically diagnosed FH, attending lipid clinics in Edinburgh (72), Newport (158), Walsall (30) and Southampton (150), were screened for the mutation. Five individuals tested positive as heterozygotes, one from Edinburgh, three from Newport and one from Southampton. This finding was confirmed by DNA sequence analysis. We conclude that FH due to this mutation occurs in individuals throughout Great Britain and that it can be detected accurately using this simple technique. DNA from these and other individuals previously identified to be heterozygous for FH E80K, was then studied using PCR of highly informative microsatellite markers flanking the LDLR gene. Sixteen of 17 apparently unrelated individuals heterozygous for FH E80K also were heterozygous for an identical size (239 nucleotide) allele, of polymorphic microsatellite D19S394, located approximately 250 kb away from the LDLR gene. This supports the hypothesis that FH E80K in these 16 individuals arose from a single ancestor less than 1000 years ago.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Base Sequence
Female
Founder Effect*
Haplotypes
Heterozygote
Humans
Hypercholesterolemia / drug therapy
Hypercholesterolemia / epidemiology
Hypercholesterolemia / genetics*
Male
Microsatellite Repeats
Molecular Sequence Data
Mutation*
Pedigree
Polymerase Chain Reaction / methods*
Receptors, LDL / genetics
United Kingdom

Substances

Receptors, LDL